J. Med. Chem. 1993,36,4195-4200
4196
Synthesis and Cytotoxicity of Potential Tumor-Inhibitory Analogues of Trimelamol (2,4,6-Tris[(hydroxymethyl)methylamino]-1,3,5-triazine)Having Electron-Withdrawing Groups in Place of Methyl Michael Jarman,' Helen M. Coley, Ian R. Judson, Timothy J. Thornton,' Derry E. V. Wilman, George Abel,t and Christine J. Rutty Drug Development Section, The Institute of Cancer Research, 15 Cotswold Road, Belmont, Sutton, Surrey SM2 5NG, U.K. Received July 6, 1993. In exploring the structural features which determine the antitumor activity of 2,4,6-tris[ (hydroxymethyl)methylamino]-1,3,5-triazine(trimelamol, 11, we have synthesized analogues in which the methyl groups have been replaced by the electron-withdrawing substituents 2,2,2trifluoroethyl(5), propargyl(13),and cyanomethyl (15) via the respective tris(alky1amino)triazines 3,12, and 14. Three mono[(hydroxymethyl)aminoltriazines (4,7, a n d 10) were also prepared. All the new tris(hydroxymethy1) derivatives showed cytotoxicities toward a variety of experimental rodent and human ovarian tumor cell lines similar t o those shown by 1,the cyanomethyl analogue (15) having the most favorable profile. Mono(hydroxymethy1) derivatives (4 and 7) were ca. onethird as toxic. T h e new tris(hydroxymethy1) analogues were more stable to aqueous hydrolysis than was 1. Half-life (pH 7.5) values were, for 1,120 min, for 5,690 min, for 13,450 min, and for 15,275 min, but a t p H 2.0,15 (tip 350 min) was the most stable. This cyanomethyl analogue was also the most water-soluble, being comparable to 1 whereas 5 and 13 were poorly soluble. 2,4,6-Tris [(hydroxymethyl)methylaminol-1,3,5-triazine (trimelamol, 1) is a third-generation analogue of hexamethylmelamine having potential advantages over the parent drug. Hexamethylmelamine is clinically active, R \N/
I 1, R
I
I
9
9
R'
9
9
C y C l N , R'
11. R
H
9 9
ChCFj CqCICH
CbOH
13. R = C & C a C H . R'
15, R
2, R
Me, RI 9 H CI+CFj. R' 9 H CH&Fj.
I
H
CHIOH
5. R 6. R
F
cH20R'
9
9
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H
particularly against ovarian carcinoma but causes severe nausea and v0miting.l It was hoped that the greater aqueous solubility of an analogue pentamethylmelamine would permit systemic administration, avoiding the side effects associated with oral hexamethylmelamine. However, pentamethylmelamine showed no significant antitumor activity in patients in a number of phase I trials (ref 2 and references cited therein), despite having activity in a number of preclinical models including human lung tumor ~ e n o g r a f t s .Metabolism ~~~ studies demonstrated a requirement for metabolic activation to cytotoxic N-(hydroxymethyl) derivatives.5 However, whereas this occurs readily in mice, cytotoxic levels of these metabolites are never achieved in patienh6 These findings prompted the development of 1,in which the requirement for metabolic activation is circumvented. In the phase I clinical trial, ~~~
* To whom enquiries should be addressed.
'Present address: Hafslund Nycomed Pharma AG, A-4021 Linz, Austria. Deceased 8 March 1993. e Abstract published in Aduance ACS Abstracts, December 1, 1993.
*
1proved less emetic and less neurotoxic than pentamethylmelamine and showed significant activity in patients with ovarian tumors resistant to cisplatin.7 These exciting findings prompted further studies designed to enhance the clinical utility of l. However, pharmacokinetic analysis has shown 1to have a very short plasma half-life in humans (6.3 f 0.6 minIe7 An approach to improved therapy with this class of compound would be the design of analogues in which the hydroxymethyl functions are stabilized. Although improved stability in aqueous solution might not have a profound effect on the half-life in uiuo, it would allow the drug to be administered by prolonged infusion. Preclinical data using the ADJ/ PC6 tumol.8 and data from the phase I clinical trial of l7 suggest that prolonged exposure would result in an enhanced therapeutic index. A more stable analoguemight also be easier to formulate, difficulty with formulation being a major obstacle to the further clinical development of 1. Stabilization could, in principle, be achieved by the use of electron-withdrawing functions in place of the methyl groups in 1. We report here the preparation of hydroxymethyl derivatives and intermediates to these containing the trifluoroethyl (2-101, propargyl (11-13), and cyanomethyl (14 and 15) functions, the aqueous stabilities and solubilities of the hydroxymethyl derivatives, and their cytotoxicities toward a variety of tumor cell lines in vitro. Whereas trifluoroethyl is a more lipophilic substituent than methyl, the respective calculated A valuesg being +1.34 and + O S , the value for cyanomethyl (-0.57) indicates it to be less lipophilic than methyl. This could be important, because it is possible that the greater CNS effecta observed clinically for pentamethylmelamine compared with 1 could be related to their relative lipophilicities.7 Low lipophilicity could therefore be a desirable feature in an analogue of 1. It is also important to establish the requirement for polyfunctionality in this class of compound. So far, the only compounds with less than three hydroxymethyl groups for which biological data have
QQ22-2623/93/1836-4195$Q4.QQIQ 0 1993 American Chemical Society
4196 Journal of Medicinal Chemistry, 1993, Vol. 36, No. 26 A
yH
R'\N/
"OH
Jarman et al. Table I. Cytotoxicities of 1 and Analogues against Various Cell Lines in Vitro ICs0 (/.M corn- Walker pound 256
I
R'
I
R'
I
H
I
H
1 4 5 6 7 13 16
PC6
H69
L1210
GCT
GCT/ CisR
9.4(0.5P 12.9(2.7) 8.5(2.3) 33.4(7.3) 24.3(0.9) 30.9(3.0) 22.5(1.5) 77.6(5.2) 42.3(3.5) 83.2(7.4) NDb ND 12.2(1.0) 29.5(4.5) 12.8(3.2) 55.1(12.5) ND ND ND 29.8(5.6) 13.4(2.0) ND 25.8(1.8) 23.7(0.3) 27.5(1.0) 71.4(17.7) 32.2(3.0) 112.5(7.8) ND ND 14.1(5.0) 35.2(5.5) 13.1(1.5) 47.8(7.1) 53.9(9.8) 47.3(4.0) 7.5(0.4) 19.4(2.0) 11.8(2.0) 32.4(0.8) ND ND
Figures in parentheses denote the standard deviations obtained for three to six replicate analyses. ND, not done.
been obtained also contain methyl group^,^ which could be metabolized to hydroxymethyl functions, leading to ambiguity in interpreting the data. The synthesis of analogues which enable this question to be addressed also forms part of the present study. Results and Discussion Synthesis of Analogues. The starting material for the synthesis of 1, namely 2,4,6-tris(methylamino)-1,3,5triazine, is made by reaction of cyanuric chloride with aqueous m e t h ~ l a m i n e . Even ~ with this relatively basic amine (pK, 10.66) displacement of all three chlorine substituents required elevated temperature. The use of both cyanuric chloride and cyanuric fluoride for the synthesis of monochlorolO and monofluorol' derivatives containing one trifluoroethylamino group only has been reported, but no derivative with more than one such substituent has been reported. We anticipated that the use of the weakly basic trifluoroethylamine (PKa 5.59) in their synthesis would certainly require the more reactive cyanuric fluoride as coreactant.12 The bis(2,2,2-trifluoroethy1)amino derivative (2) was conveniently prepared by mixing the reagents in the absence of solvent. Displacement of the third fluorine substituent proceeded smoothly in DMF when cesium fluoride was added to give the required intermediate tris((2,2,2-trifluoroethyl)amino)triazine (3). Alternatively, 3 could be prepared in more modest yield by conducting the reaction (without CsF) in refluxing toluene. The reaction between 3 and 40 % aqueous formaldehyde adjusted to pH 8.9, conditions we have used to prepare 1 from trimethylmelamine, gave only a mono(hydroxymethyl) derivative (4). The introduction of further hydroxymethyl substituents required the addition of the stronger base KzC03. However, the product which separated from the reaction mixture under these conditions was not the desired tris(hydroxymethy1) analogue (5) but was compound 6, having one of the hydroxymethyl groups modified by further reaction with formaldehyde. This (hydroxymethoxy)methyl derivative was, however, readily and virtually quantitatively converted into the desired compound 5 by treatment with aqueous acetone. The formation of an N-(hydroxymethoxy)methyl derivative has a precedent in the literature. 2',3',5'-Tris(acety1arabinosylladenine afforded its 6- [ [(hydroxymethoxy)methyllaminol derivative on reaction with aqueous formaldehyde.13 The availability of 2 made possible the preparation of an analogue (7) of mixed functionality. First 2 reacted with methylamine, the stronger base here catalyzing its own displacement of the remaining fluorine substituent,
and the intermediate (8) then reacted with formaldehyde to form a mono(hydroxymethy1) derivative (7) analogous to 4. The lH-NMR spectrum of 7, when compared with those of 3-5, together with the presence of two fluorine signals in the IgF-NMR spectrum clearly showed that the hydroxymethyl substituent was contiguous with trifluoroethyl and not with methyl. Finally, the known1' reaction of cyanuric chloride with 2,2,2-trifluoroethylamineintroduces a single trifluoroethylamino substituent, and subsequent reaction with dimethylamine gave an intermediate (9) from which a further mono(hydroxymethy1) derivative ( 10) was prepared. Propargylamine (pK, 8.15) is also a much weaker base than methylamine, and cyanuric fluoride was again the preferred coreagent, analogously yielding the monofluoro bis(propargy1amino) derivative (11) and the tris(propargylamino) derivative (12). The latter could also be prepared, albeit in modest yield (32% us 93%), from cyanuric chloride. The reaction of 12 with formaldehyde to form a tris(hydroxymethy1) derivative (13) again required addition of KzC03. However, its omission did not yield a mono(hydroxymethy1) derivative instead: it simply prevented the separation of any product from solution. The tris((cyanomethy1)amino)triazine 14, a potential precursor to the corresponding analogue (15) of 1, has been prepared in an impure form in two steps starting from aminoacetonitrile and cyanuric ch10ride.l~ In our hands the reaction with cyanuric chloride was unsatisfactory, but the reaction with cyanuric fluoride in DMF gave pure 14. Although the pK, values of aminoacetonitrile (5.34) and trifluoroethylamine (5.59) are similar, addition of CsF was not necessary in the formation of 14. The formation of the analogue 16 in contrast to that of 6 or 13 proceeded without addition of base and without precipitation of the product from the reaction mixture. In Vitro Cytotoxicities. The data shown in Table I indicate the activity of (hydroxymethy1)melamine analogues containing electron-withdrawing groups compared with 1. In the trimelamol-sensitive cell lines Walker rat carcinoma 256 and the human small cell lung cancer H69, the analogues 5,6,13, and 15 show activity similar to that for 1, as seen from the IC50 values in Table I. Compound 15 appears the most promising in this respect. Again, in the trimelamol-sensitive ADJ/PC6 murine plasmacytoma cell line, compound 15 appears the most cytotoxic of the analogues tested, with somewhat higher IC50 values being obtained for compounds 5,6, and 13. In the L1210 murine lymphocyticleukemia cell line, again 15 shows the closest activity to that of 1. The use of GCT/GCTCisR cell lined5with intermediate sensitivity to 1 provides evidence for the effectiveness of
Potential Tumor-Inhibitory Analogues of Trimelamol
Journal of Medicinal Chemistry, 1993, Vol. 36, No.26 4197
Table 11. Half-Life ( t 4 in min for Tris(hydroxymethy1) Derivatives in Water at Varying pH at 37 "C compound pH 7.5 pH 5.0 pH 2.0 1 120 200 ND 5 690 ND 60 13 450 ND 40 15 275 960 350
Table 111. Half-Life (t14 in min for Tris(hydroxymethy1) Derivatives in Various Media at Room Temperaturea compound medium 1 5 15 water pH 5.0 820 NDb 6120 water pH 7.5 ND 5100 4510 0.9% sodium chloridec 275 5700 8090 5% dextrosed 350 3000 10800 Room temperature 20-24 O C . ND, not done. pH sodium chloride solution = 5.2. pH dextrose solution = 4.0.
1 and analogues against cis-platinum resistant human ovarian carcinoma cell lines. The IC50 values obtained in both cell lines indicate resistance factors of 1.3 and less for the three compounds tested. Clearly those compounds containing three hydroxymethylgroups, Le. 5,13, and 15 (and 6, which is a pro-drug for 5), have superior cytotoxic activity over those compounds containing only one such group, i.e. 4 and 7, for all the cell lines tested. The cytotoxic activity of either 4 or 7 varied from 3- to 6-fold less than that of 1, as indicated by IC50 values. Stability Studies. The influence of the trifluoromethyl substituent on the stability of the hydroxymethyl function under simulated physiological conditions was determined first, by comparing compound 10, containing contiguous hydroxymethyl and trifluoroethyl functions, with N-(hydro~ymethy1)pentamethylrnelamine.~ The t 1 p values for the release of the respective products 9 and pentamethylmelamine in human plasma a t 37 OC were respectively 45 and 30 min. Hence, replacement of methyl by trifluoroethyl does give a useful degree of stabilization which should be enhanced by multiple substitution. The stabilities of the tris(hydroxymethy1) analogues and 1 were compared in aqueous solution a t 37 "C (Table 11). At approximately physiological pH, all analogues show superior stability over that for 1. The trifluoroethyl analogue 5, showing a 4-fold increase in stability, appears the most stable compound a t this pH. The rankings of 5 and 13 a t this pH were as expected from their relative electron-withdrawing effects reflected in the pKa values of the appropriate amines. The reason for the surprisingly lower stability of 15 a t this pH requires further explanation. On the basis of mechanisms previously proposed16for the loss of formaldehyde from 1, an acid-catalyzed mechanism in which exocyclic nitrogen is protonated and a basecatalyzed one in which the hydroxyl group is ionized, the electron-withdrawing substituents in the new analogues should be stabilizing a t acidic pH values but destabilizing a t alkaline pH. These mechanisms account for the relative stabilities of these compounds a t pH2. Indeed, the stability of compound 15 a t this pH would appear to offer the possibility of an oral route of administration. However, to explain the rankings a t pH 7.5, one must suppose that the base-catalyzed mechanism is promoted a t this pH value only by the most electron-withdrawing substituent, namely cyanomethyl. Lastly, studies of stability a t ambient temperature (Table 111) afford data which indicate the likely stability of compounds under conditions of continuous infusion and again show 1 to be the least stable compound. Solubility Studies. The solubility of 1 has been previously quoted3 as 9.04 mg/mL from measurement of UV absorption. The experimental procedure employed to obtain this result, however, would undoubtedly have caused extensive degradation of the compound and should therefore be regarded as unrealistic. The material used in the present study was a ball-milled and lyophilized preparation used in the clinical trial of 1.' Solubilities for
~~
Table IV. Aqueous Solubilities of Tris(hydroxymethy1) Derivatives compound solubility (mg/mL) 1 4.50 5 0.03 13 0.03 15 1.0 a Lyophilized, ball-milled material. ~~
5 and 13 were low whereas that for 15 is a t an acceptable level to consider it as suitable for iv formulation (Table IV). The solubility of 15 has been shown to be further enhanced by lyophilization and by solubilization in PEG 400 solution (data not shown). In summary, whereas the data shown in Tables I1 and I11 demonstrate the superior stability for compounds 5, 13, and 15 over that seen for 1, considerations of solubility make 15 the preferred candidate for further development as a potential improvement on 1.
Experimental Section Chemical Synthesis. 'H- and lBF-NMRspectra were determined with a Bruker AC 250 spectrometer with MedSi and C$e, respectively, as internal standards. The determination of HPLC retention times was conducted using a 15 cm X 4.6 mm stainless steel column packed with Spherisorb S5 ODS2. Detection was at 254 nm, and a Trilab I11 (Trivector, Sandy, Beds., England) was used for data processing. Infrared spectra were determined with a Perkin-Elmer 1720X spectrometer. Mass spectra were determined using a VG 7070H spectrometer and VG 2235data system. Electron impact (EI)spectra were obtained at an ionizing voltage of 70 eV and ion-sourcetemperature of 150 "C, and chemical ionization (CI) spectra at 50 eV with methane as ionizing gas. Fast atom bombardment (FAB)mass spectra were carried out using the Iontech saddle field gun which directed fast atoms of xenon (6 kV) at the matrix on a stainless steel probe tip. Melting points were determined on a Kofler block (Reichert Thermovar) melting point apparatus and are uncorrected. Elemental analyses were determined by CHN Analysis Ltd., South Wigston, Leicester, England. 2-Fluoro-4,6-bis[ (2,2,2-trifluoroethyl)amino]-1,3,5-triazine (2). To cyanuric fluoride (1.62 g, 12 mmol) was added with stirring at 0 "C 2,2,2-trifluoroethylamine(3.17 g, 24mmol).When the initially vigorous reaction had subsided, the mixture was placed under vacuum (rotary evaportor) to remove excess reagents. The resulting white solid (3.41 g, 97 %) gave colorless crystals from EtOAc: sub185 OC; m/z 293 (M+,56%1,274 (40%), 273 (52%),and 224 (100%). Anal. (C7HeF7Nd C, H, F, N. 2,4,6-Tris[ (2,2,2-trifluoroethyl)amino]-l,3,5-triazine(3). (a) In Dimethylformamide. To a stirred solution of cyanuric fluoride (2.025 g, 15 mmol) in dry DMF (12.5 mL) was added through a septum attached to the top of a reflux condenser 2,2,2trifluoroethylamine (7.45g,75mmol). When theinitiallyvigoroue reaction had subsided, CsF (5 g) was added and the mixture stirred at 40 "C for 3 days. The slurry was then poured onto ice (100 g), and 3 was recovered as a white solid (5.08 g, 91% ) after washing with ice-cold water and desiccation: 6~ (CDCls)4.05 (m, 6, CH2), 7.41,7.57 (2 br s,3, NH); 6~ -70.3 (8, CFs); mlz (EI)372 (M+). This product was used directly for the preparations of 4 and 5.
Jarman et 41.
4198 Journul of Medicinal Chemistry, 1993, Vol. 36,No. 26
3.09 h 1 2 , CHa), 4.10 (m, 2, CHzCFa), 4.89 (br t, 1,NH); Sp-73.2 (b) In Toluene. To a stirred solution of cyanuric fluoride (t, J p ~ = i 9.4 Hz, CFa). Anal. (C&Hl$&) C, H, N. (1.56 g, 0.85 mL, 11.53 m o l ) in dry toluene (50 mL) was added 2&Bi~(d h e th~lamin0)-6-[ ( h y d r o m h y l )(2ff-trlll~2,2,%trifluoroethylamine (6.89 g, 69.2 mmol). When the initidly oroethyl)aminol-lPPtriazine(10). A saturated solution of vigorous reaction had subsided, the mixture was heated under 9 (300mg) in H2O (1600 mL) and 0.1 M NaOH (10 mL) was reflux for 20 h. Solid was removed by fitration and the fitrate concentrated. Crystallizationof the residue fromHOAc (25mL)/ prepared by overnight stirring at room temperature. Further 0.1 M NaOH (10 mL) was added to the fitered solution to bring HzO(20mL)afforded3(2.24g,52%):mp73-75OC;NMRepectra identical with the product from section a above. And. the pH to 10.5; then 40% aqueous formaldehydeadjusted to pH 8.5 (25 mL) was added to give a f i pH of 10 and the mixture (C9Hga6) C, H, F, N* 24( H y ~ x ~ e t h y l ) ( 2 , 2 f - t r i i l u o r o e t h y l ) ~ o ] - 4 , 6 - b i s - stirred overnight,whereupon 10 separated an a white solid which was recovered by washing with ice-cold water and air drying (SO [(~~~-trifluoroet~l)amino]-lf~triaeine (4). A mixture of mg):mp 101-103 OC. Anal. (CloH&&&H&) H, N. Found 3 (744 mg,2 mmol) and 40% aqueous formaldehyde adjusted to C, 38.00%. Required: C, 38.46%. pH 8.9 (7.5 mL) was stirred for 16 h. Following complete dissolution of starting material, 4 separated subsequently and 2-Fluoro-4,6-bis(propargylamino)-lf,S-triadne(11). To was recovered as a white solid (585mg,73% ) after washing f i t a stirred solution of cyanuric fluoride (810 mg,6 mmol) in dry with the formaldehydesolution and then with ice-cold water and DMF (5 mL) was added propargylamine (660 mg, 12 mmol). After the initial reaction had subsided, further propargylamine then desiccation at 5 OC. Recrystallization from CH2Cl2 gave colorleascrystale(445mg)havingaretentiontime(HPLC,MeCN/ (330 mg, 6 mmol) was added. When the further reaction had aqueous NWCOa, 1:l)of 1.7 min: subl 135OC; 6~ (MefiO-dd subsided, 11had separated as a white solid (333 mg): subl 157 OC; m/z (CI) 206 ([M + HI+, 100%). Anal ( W N d C, H, N. 4.06 (app t, 4, NHCH~CFI,slight sharpening on D20 shake to Found F, 8.55 % Required: F, 9.26 % . Further product wan app q), 4.41 (q, J = 9.5 Hz,2, CH2NCH&F3), 5.07 (d, J = 6.3 Hz, recovered from the fitrate by precipitation with water (20 mL), 2, CHzOH, s on D20 shake), 5.74 (t, 1, OH), 7.69 (br 8, 2, NH); making a total yield for 11 of 1.076 g (87%). Sp -68.4 (app 8,3, CH&ICH&Fs), -70.32 (app s,6, NHCH2CFa) ;m/z (FAB, matrix PEG) 403 ([M + HI+, 35%), 385 ([M + H 2,4,6-Tris(propargylamino)-l,3~t~~ne (12). (a) From - HzOl*, 100%), 373 ([M + H - CH201+, 68%). Anal. Cyanuric Fluoride. To a stirred solution of cyanuric fluoride (CldI11F&o) C, H, Ne (1.35 g, 10 mmol) in toluene (20 mL) was added a solution of propargylamine (3.30 g, 60 mmol) in toluene (30 mL) during 5 2,4,6-Trir[(hydroxymethyl)(2,2,2-trifluoroethyl)amino]min. The mixture was heated under reflux for 3 h and then 1,3$-triazine (5). To a stirred solution of KzCOa (829 mg,6 filtered hot. The fitrate deposited 12 as pale buff crystale (2.225 mmol) in 40% aqueous formaldehyde adjusted to pH 8.9 (20 g, 93%) of retention time (HPLC, MeCN/aqueous "COa, mL) was added 3 (2.231 g, 6 mmol) prepared by method a. The 7:3) 1.8 min: mp 125-127 "C; v,. ( f ifrom CH&12) 2116 cm-' mixture wan stirred for 3 days, and the resulting white solid was (C=C str), 4.17 (br 8, 6, CHd, 5.04 (br 8, 3, NH). recovered by fitration, washed with aqueous formaldehyde and then with ice-cold water, and dessicated at 5 OC to give (b) From Cyanuric Chloride. To a stirred suspension of 2-[((hydroxymethoxy)methyl)(2,2,2-trifluoroethyl)amino]-4,6cyanuric chloride (1.84 g, 10 mmol) in dry toluene (50 mL) was his[ (hydroxymethyl)(2,2,2-trifluoroethyl)amino]-l,3,5-t~e (6; added dropwise,during 5 min,propargylamine(3.30 g, 60-01). 1.81 g, 61%): 6~ (MezS0-A) 4.45 (br q, 6, CHzCFs), 4.65 (d, 2, When the initial reaction had subsided, the mixture was heated J = 7.6 Hz,OCHsOH), 5.06 (br t, 4, NCHzOH), 5.21, 5.25 (a, under reflux for 20 h and then fitered hot. The solid which total 2, NCH20CH20H), 5.90 (2t,2, NCHzOH), 6.39, 6.59 (2t, separated on cooling was removed by filtration, the fitrate wan total 1,J = 8.5 Hz, OCHflH); Sp -67.9, -68.1 (2t, HOCHzOCHr concentrated, and the residue was r e c r y s t d i d from boiling NCHzCFa),-68.5 (m, HOCH2NCH2CFa). Anal. (CisHi,FsNsO4) water to give 12 (773 mg,32%) as colorlees rods identical with C, H, N, F. A solution of 6 (1.66 g, 3.59 mmol) in acetone (10 mL) material prepared from cyanuric fluoride. Anal. (C12HuNs) C, was treated with water (6.66 mL) and then set aside for 1h at H, N. room temperature. Acetone was removed under vacuum, and 2,4,6-Trie[ (hydroxymethyl)propargylamino]-l,3~triazthe resulting white precipitate, recovered by filtration, washed ine (13). To a stirred solution of K2CO3 (414 mg, 3 mmol) in with water, and dried under vacuum over CaCL, was the title 40% aqueous formaldehyde adjusted to pH 8.9 was added 12 compound 5 (1.54 g, 99% from 6): 6~ (Me2SO-dd 4.45 (2 (240 mg,1mmol). Complete dissolution occurred in 2 h. After 3, OH); overlappingq, 6, CH~CFI),5.06 (2d, 6, CH20H),5.87 (a, 3 days 13 had separated and was recovered by fitration (caution: 6p -68.4 (m, CH2CFs). Anal. C, H, F, N. the product is somewhatgelatinous),washing f i t with aqueous 2-[(Hydroxymethyl)(~~-trilluoroethyl)~o]-4(meth- formaldehyde and then with ice-cold water, and then drying in ylamino)4-[ (2,2,2-trifluoroethyl)amino]-l,3$-triazine (7). vacuo at 5 OC as a white solid (251 mg,76%) of retention time A mixture of 2 (2.34 g, 8 mmol) and 30% aqueous methylamine (HPLC, eluant as for 12 above) 1.5 min: Y- ( f ifrom CH&ld (40 mL) was stirred for 16 h. The supernatant was decanted 2115 cm-'(Wstr); 6~ (CDCL) 2.25 (t, J = 2.5 Hz, 3, W H ) , from the oil which separated and was then stirred with H20 (50 4.39 (br s, 6, W C H 2 ) , 5.13 (8, 6, HOCH2); m/z (FAB, matrix mL), and the process was repeated. After two further additions m-nitrobenzylalcohoVPEG)331([M+ HI+). AnaL (C~sHteNsOa) of H2O and decantation, the oil was triturated with icewater, C, H, N. whereuponcrude 2-(methylamino)-4,6-bi[(2,2,2-trifluoroethyl)2 , ~ 6 - T r i ~ [ ( ~ y a n o m e t h y l ) a m i n o ] - l f ~(14). t M ~A SU& amino]-1,3,5-triazine (8) was obtained as a white solid which pension of aminoacetonitrilehydrochloride (9.25 g, 0.1 mol) and upon fitration and vacuum desiccation afforded a hygroscopic NdCO3 (42 g, 0.5 mol) in dichloromethane (150 rnL) was glass (1.26 g, 52%,m/z304 (M+,100%))which was used without vigorously stirred for 16 h. Solid was removed by fitration, and further purification to prepare 7. A mixture of 8 (304 mg, 1 the filtrate was concentrated at 50 OC on a rotary evaporator to m o l ) and 40% aqueous formaldehyde adjusted to pH 8.9 (5 give aminoacetonitrile as a mobile, colorless oil (4.62 g, 82%): mL) was stirred for 1h, whereupon 7 separated during 24 h as 6~ (DMSO-&) 6 2.05 (br s, 2, "I), 3.48 (8, 2, CHd, 5.73 (8, a white solid (446mg,51% ): 6~ (Me&O-ds) 2.75 (e, 3, CHI), 4.07 integration0.7% ofsignalat63.48,reaidualCH&ld. Toastirred (br s,3, HNCH&Fs), 4.40 (m, 2, HOCH~NCH~CFS), 4.84 (d, 2, solution of cyanuric fluoride (2.025 g, 14 m o l ) in dry DMF (15 CH&H), 5.74 (m, OH), 7.00 (m, 1, "CHI), 7.64 (m, 1, NHCHr mL) in a flask surrounded by an ice bath was added dropWiae CF&&-69.4 (apps,3,CH&ICH2CF3),-71.2(apps.3,HNCHr through a septum by syringe aminoacetonitrile(5.89 g, 105mm01, CFa). Anal. ( W W " s O ) C, H, F, N. 7 mol equiv), generated by the foregoingmethod, during 5 min. The cooling bath was removed and the reaction mixture stirred 2,4-Bis(diithylamino)-6-[(2.2,2-trifluoroethyl)amino]at ambient temperature for 3 h and then treated with ice-cold 1,3&triazine (9). A solution of 2,4dichloro-6-[(2,2,2-trifluowater (150 mL). The resulting white solid was recovered by roethyl)amin0]-1,3,5-triazine~~(3.1 g, 0.013 mol) in aqueous filtration and washed with water, and the still moiet solid was dimethylamine (25% w/v, 200 mL) was heated under reflux, f i t recrystaked from boiling water (200 mL), a small insoluble alone and, then when TLC indicated incomplete reaction, with residue being removed by filtration of the hot solution, to yield additionof NaOH (1.2 g,0.03 mol). The solid obtainedon fitering 14 as colorless needles (2.778 g, 76%): mp 232-234 OC (lit." mp the cooled reaction mixture was recrystallized from light petro216-228 OC for analyticallyimpure compound). 6~ (CDCb)4.21leum(bp60-8O0C)toyield9(1.8g,52%): mp 1oooc;6H (CDC13)
.
Potential Tumor-Inhibitory Analogues of Trimelamol
Journul of Medicinal Chemistry, 1993, Vol. 36, No.26 4199
4.33 (m, 6, CHZ),7.59-7.87 (m, 3, NH); m/z 243 (M+;79%),189 ([M - NCHzCN]+, 71%). Anal. (CgHgNg) C, H, N. 2,4,6-Tris[ (cyanomethyl)(hydroxymethyl)amino]-1,3,5triazine (15). 2,4,6-Tris[(cyanomethyl)aminol-1,3,5triazine (14, 2.432 g, 10 mmol) was added to 40% aqueous formaldehyde (50 mL) (unbuffered, measured pH = 4.0), and the suspension was stirred at ambient temperature for 3 days. The now clear solution was extracted with ethyl acetate (150mL and then 100mL), the combined extracts were dried over NazSOd and concentrated, and the residual clear syrup was triturated with water (50 mL) to give a white crystalline solid, recovered by fitration, washed with water, and dried in uacuo over CaCh, which was the hemihydrate of 15(1.804 g, 53%): 6~ (MezSO-de)4.61 (e, 6, CH2CN), 5.12 (br d, 6, CHzOH, J = 6.2 Hz), 5.95 (br s, OH). Anal. (C~ZH~&O.YO.~H~O) C, H, N. Cell Culture. All cell lines were grown up in continuous culture. The Walker 256 carcinoma cell line was grown in Dulbecco's m i n i essentialmedium (DMEM)with the addition of 10% donor horae serum (DHS), 2 mM glutamine, and antibiotics; the ADJ/PC6 murine plasmacytoma cell line was grown up in DMEM with the addition of 20% DHS, 2 mM glutamine, antibiotics, hydrocortisone (0.5 pg/mL), and insulin (10 pg/mL) (Sigma, Poole, Dorset, UK). The human small cell lung cancer cell line H69 was grown up in RPMI medium with 10% fetal calf serum (FCS), 2 mM glutamine, and antibiotics. The L1210 murine leukemia cell line was grown up in RPMI medium with 10% DHS, glutamine, and antibiotics. The human testicular cell lines GCT-27 and GCT-27/CisR were grown up in DMEM plus 10% FCS, glutamine, antibiotics, hydrocortisone, and insulin (as for ADJ/PC6). All cell culture media and supplementswere obtained from GibcoLife Technologiesunless otherwise stated. Cell cultures were periodically checked for the presence of mycoplasma, all cultures used in the study being free from infection. Cytotoxicity Testing. The MTT assay used was essentially that degcribedby Mosmann,lewith a number of modifications.17J8 All cell lines apart from the GCT cell lines grow as suspension cultures. Prior to seedingonto 96 well tissue culture plates (Nunc, GibcoLife Technologies,Paisley, Scotland),suspension cultures were reduced to a single cell suspension (either by repeated pipetting or syringing through a 19-gaugeneedle). The GCT cell lines were harvested by trypsinization (0.02 % EDTA/O.O5 % trypsin; Gibco Life Technologies, Paisley, Scotland) and then reduced to a single cell suspension by syringing as above. Cells were plated at between 1X 109and 8 X lo3cells per well in a 200-pL aliquot. Drugs were initially diluted in DMSO and stored as frozen aliquota which were thawed immediately before use and diluted in tissue culture medium. Cellswere drug treated in continual exposure. The 96 well plates were left for between 72 and 144h according to the respective growth rates of the different cell lines (aa measured by doubling times), at 37 OC and 8% COZ in a humidifying incubator. Following this incubation period, M'M' (Sigma, Poole, UK) solution (5 mg/mL in phosphate buffered saline) was added to each well in a volume of 20 pL. Plates were further incubated between 4 and 5 h at 37 OC. The formation of formazan crystalswas terminated by removal of supernatent from each well by centrifugation of plates containing suspension cultures (300 g for 5 min) followed by removal of supernatent by aspiration. The crystalline deposit of M" formazan was then dissolved in 200 pL of DMSO and allowed to agitate gently for 10 min. Absorbances were read on a Titertek Multiskan ELISA plate reader (Flow Laboratories, Helsinki, Finland) at a wavelength of 540nm (with a reference wavelengthof 690 nm). The absorbance values obtained were expressed aa a fraction of those obtained for the control untreated wells. In all experiments 3-6 replicate wells were used for each drug concentration. Each assay was carried out at least twice. Stability Studies (i). Decomposition of 10 in Human Plasma. To fresh human plasma (9.9 mL) maintained at 37 OC was added a solution of 10 (0.1 mL; 10 mg/mL) in dimethyl sulphoxideto give a fimal concentration of 100pglmL. At intervals of 0,5,10,15,20,30,40,50,60,75,90,105, and 120 min, aliquota (0.5 mL) were withdrawn and added to ice-cold MeOH (1mL).
After centrifugation at 4 "C the supernatants were placed in cooled vi& on a cold plate (3 "C) and aliquots (25pL) analyzed by HPLC using an autosampler. The column used was a C6 (Spherisorb) 15 cm X 4.6 mm with a precolumn and was eluted with MeOH/O.O5 M aqueous NHSICOa, 5545, at a flow rate of 1.5 mL min-I. Products were monitored by absorbance at 225 nm. Retention times were, for 10,ll.Omin and, for ita breakdown product 9,9.6 min. By an essentially identical procedure, but using MeOH/40% aqueous ammonium formate, 6040, as eluant and a flow rate of 1 mL min-I, the breakdown of N-(hydroxymethy1)pentamethylmelamine to pentamethylmelamime (respective retention times 12.65 and 5.45 min) was studied. Stability Studies (ii). Decomposition of Compounds 5, 13, and 15 in Various Media. The stability of compounds 5, 13,and 15was measured by HPLC analysis. Stock preparations of compounds were made by dissolving in DMSO to a concentration of 50 mM. Aliquots (10 mL) of the appropriate medium were dispensed into polypropylene test tubes followed by the addition of drug solutions to a final concentration of 100 pM. Both 37 OC and ambient-temperatureincubation conditions were controlled by incubation of test tubes in water baths. HPLC analysis involved the use of a 15 cm X 4.6 mm steel column packed with C8 octyl5-pm Spherisorb material (Phase Sep,Deeside,UK),with precolumn, which affordedthe separation of all compoundsin the study. In the case of 1an isocraticmethod using 90% 0.05 M ammonium bicarbonate (pH 8.1) in HPLC grade 'Hypersolv' water (BDH) and 10% acetonitrile (Romil Chemicals,Loughborough, U.K.) mobile phase was employed at a flow rate of 1.5 mL/min. Separation of 15 from products of decomposition was also achieved isocratically by the foregoing 10% acetonitrile mobile phase at a flow rate of 1.5 mL/min. Separation of 5 and 13 from their products involved a gradient elution using 30% acetonitrile in 0.05 M ammonium bicarbonate running into 60% acetonitrile in 0.05 M ammonium bicarbonate over a period of 10min with a flow rate of 2 mL/min. The column was housed in a cooling cabinet maintained at a temperature of 15-17 OC. Peak detection was by UV absorbance at 225 nm for all compounds. The Perkin Elmer ISS-100 sample injector module with refridgeratedsample plate was set at a samplevolume of 10 pL. Half-life (tip) calculationswere based on the decrease in peak area from the HPLC chromatogram with time. Peak areas were computed by on-line link with the MT2 450 data acquisition system (Kontron Instruments, Watford, U.K.). Half-life values were calculated from semilog plots of peak area (y) against time ( x ) . All measurements were performed on at least two different occasions,with avariation from between 2 and 22 % . Throughout the period of analysis preparations of known concentrations of the compound of interest were run as a control for any shift in retention time and/or change in the standard curve calibration. Measurement of Aqueous Solubility of Compounds 5,13, and 15. Each compound (approximately 30 mg) was placed in a small glass stoppered vial. Deionized water (2 mL) was then added and the solution placed in water in a sonication bath. During this period the temperature of the bath water was maintained around 15 "C by periodic addition of iced water. This eliminated any excessive degradation of the compounds under study. The glass stoppered vials were then centrifuged at 2000 rpm for 5 min. The supernatent was then drawn off and recentrifuged to ensure the elimination of all particulate matter. Supernatants were then analyzed by HPLC according to the methodology described under Stability Studies (ii). Peak areaa obtained were then read off a standard curve and calculated as solubility in mg/mL (Table IV).
Acknowledgment. This work was supported bygranta from the Cancer Research Campaign and the Medical Research Council. We also thank Sterling Winthrop Inc., Malvern, PA, for financial support (to H.M.C. andT.J.T.), Professor K. R. Harrap for his interest, Dr. L. R. Kelland for the provision of ovarian cell lines, and Mr. M. H.Baker for determining the mass spectra.
4200 Journal of Medicinal Chemistry, 1993, Vol. 36, No.26
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